首页> 美国卫生研究院文献>Journal of Anatomy and Physiology >Dual-channel laser scanning microscopy for the identification and quantification of proliferating skeletal muscle satellite cells following synergist ablation.
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Dual-channel laser scanning microscopy for the identification and quantification of proliferating skeletal muscle satellite cells following synergist ablation.

机译:双通道激光扫描显微镜用于鉴定和定量增效消融后增殖的骨骼肌卫星细胞。

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摘要

Proliferating skeletal muscle satellite cells are the source of additional myonuclei which allow skeletal muscle to grow and regenerate. Previously, proliferating satellite cells were identified in situ by techniques which were limited either by tissue processing time or inability to observe complete muscle sections, or by errors made in separating these cells from proliferating nonmyogenic cells. To overcome these problems a new method has been devised for the identification and quantification of proliferating satellite cells in situ by light microscopy. The technique involves dual-channel laser scanning imaging of whole muscle sections for the localisation of both the muscle fibre basal lamina and the cell division marker bromodeoxyuridine. Using this technique satellite cell proliferation was quantified in mouse limb muscle following synergist ablation. Dual-channel laser scanning microscopy allowed precise localisation of proliferating satellite cells in the experimental model and, after 4 d, synergist ablation was shown to have produced significant satellite cell proliferation when compared with contralateral and sham-operated controls.
机译:增生的骨骼肌卫星细胞是额外的肌核的来源,其使骨骼肌生长和再生。以前,通过组织处理时间或无法观察完整的肌肉切片,或由于将这些细胞与增殖的非肌源性细胞分离所产生的错误而受到限制的技术在原位鉴定了增殖的卫星细胞。为了克服这些问题,已经设计了一种新的方法,用于通过光学显微镜原位鉴定和定量增殖的卫星细胞。该技术涉及整个肌肉切片的双通道激光扫描成像,以定位肌肉纤维基底层和细胞分裂标记物溴脱氧尿苷。使用该技术,在协同消融后,在小鼠肢体肌肉中定量了卫星细胞增殖。双通道激光扫描显微镜可以在实验模型中精确定位正在增殖的卫星细胞,并且与对侧和假手术对照组相比,在4 d后,协同消融显示产生了明显的卫星细胞增殖。

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